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首页> 外文期刊>Human Reproduction >Ovarian tissue viability following whole ovine ovary cryopreservation: assessing the effects of sphingosine-1-phosphate inclusion.
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Ovarian tissue viability following whole ovine ovary cryopreservation: assessing the effects of sphingosine-1-phosphate inclusion.

机译:整个绵羊卵巢冷冻保存后的卵巢组织生存力:评估鞘氨醇-1-磷酸盐的作用。

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BACKGROUND: Cryopreservation is hypothesized to result in apoptosis, contributing to stromal damage and follicle loss in ovarian tissue. This study investigated tissue viability following whole ovine ovary cryopreservation and examined the effects of the anti-apoptotic agent sphingosine-1-phosphate (S-1-P) on ovarian cryopreservation efficiency. METHODS: Whole ovine ovaries were cryoperfused and subjected to slow-freeze, rapid-thaw cryopreservation before a range of functional viability tests were performed. The effects of 20 micromol(-1) S-1-P, in the cryopreservation media, were then assessed against a control cryopreservation media and non-frozen tissue. RESULTS: Granulosa cell viability (assessed by trypan blue) was not significantly affected, however, Ki67 expression, indicative of cellular proliferation, was reduced following cryopreservation (P< 0.05). Following S-1-P supplementation, granulosa cell viability was not affected by either cryopreservation or S-1-P inclusion. Bromodeoxyuridine uptake, demonstrating DNA synthesis, was seen in both cryopreserved and fresh cortical tissue and the viability stain, 5(6)carboxyfluorescein diacetate succinimidyl ester, showed many viable small follicles. Cryopreservation increased arterial endothelial disruption (P< 0.01), but not internal elastic lamina rupture or venous damage. However, S-1-P supplementation did not improve ovarian or vascular tissue survival. CONCLUSIONS: These results are encouraging for whole ovary cryopreservation, demonstrating maintained cell viability, however, they do not support S-1-P inclusion at this concentration to improve tissue viability following cryopreservation.
机译:背景:假设冷冻保存会导致细胞凋亡,从而导致卵巢组织的基质损伤和卵泡丢失。这项研究调查了整个绵羊卵巢冷冻保存后的组织活力,并研究了抗凋亡剂鞘氨醇-1-磷酸(S-1-P)对卵巢冷冻保存效率的影响。方法:对整个绵羊卵巢进行冷冻灌输,并进行慢冻,快速融化的冷冻保存,然后进行一系列功能生存力测试。然后针对对照冷冻保存介质和非冷冻组织评估了冷冻保存介质中20 micromol(-1)S-1-P的作用。结果:颗粒细胞活力(通过锥虫蓝评估)未受到显着影响,但是,冷冻保存后,Ki67表达(指示细胞增殖)降低(P <0.05)。补充S-1-P后,冷冻保存或S-1-P包埋均不影响颗粒细胞活力。在冷冻保存的和新鲜的皮质组织中均可见到溴脱氧尿嘧啶核苷的摄取,表明了DNA的合成,并且活力染色剂5(6)羧基荧光素二乙酸琥珀酰亚胺酯显示了许多可行的小卵泡。冷冻保存增加了动脉内皮破坏(P <0.01),但没有内部弹性椎板破裂或静脉损伤。但是,补充S-1-P并不能提高卵巢或血管组织的存活率。结论:这些结果对于整个卵巢冷冻保存是令人鼓舞的,表明维持了细胞的活力,但是,它们不支持该浓度的S-1-P包涵体以提高冷冻保存后的组织活力。

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